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rbcg expressing brucella melis l7/l12 gene and its construction method and application

A technology for brucellosis and brucellosis, applied in the field of rBCG expressing the L7/L12 gene of brucella melis and its construction, to achieve the effect of solving poor immune effect and saving costs

Active Publication Date: 2020-06-23
INNER MONGOLIA MEDICAL UNIV
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  • Summary
  • Abstract
  • Description
  • Claims
  • Application Information

AI Technical Summary

Problems solved by technology

[0005] At present, there is no report on the construction of recombinant BCG carrying the ribosomal protein L7 / L12 coding gene (L7 / L12 gene) of the M5 strain of Brucella melii at home and abroad.

Method used

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  • rbcg expressing brucella melis l7/l12 gene and its construction method and application
  • rbcg expressing brucella melis l7/l12 gene and its construction method and application

Examples

Experimental program
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Effect test

Embodiment 1

[0030] Embodiment 1 carries the construction of the recombinant expression vector of Brucella melii L7 / L12 gene

[0031] Include the following steps:

[0032] 1. According to the published sequence of the L7 / L12 gene of Brucella melis (GenBank: EF173477.1), after codon optimization using Jcat software, the L7 / L12 gene after the full sequence optimization was artificially synthesized as the target gene (nuclear The nucleotide sequence is shown in SEQ ID NO: 1).

[0033] 2. Construction of the recombinant expression vector carrying the L7 / L12 gene of the M5 strain:

[0034] The above target gene was inserted into the shuttle expression vector pMV361 through two restriction sites of Mun I and Pvu II.

[0035] 3. Verification of inserting the correct recombinant expression vector:

[0036] Through nucleic acid sequence determination, it was confirmed that the recombinant expression vector carrying the optimized Brucella melis L7 / L12 gene was constructed successfully.

Embodiment 2

[0037] Example 2 Construction of rBCG expressing Brucella melis L7 / L12 gene

[0038] 1. Using BCG as the host bacterium, transform the recombinant expression vector constructed in Example 1 (full sequence shown in SEQ ID NO: 2) into BCG.

[0039] The electroporation method was used for transformation, and the experimental conditions were: 2500V, 25μF, 1000Ω, electroporation time 5ms, 0.1cm electric shock cup. The electroporation reaction system is: 4 μl of plasmid (concentration is 0.51 μg / μl), 100 μl of competent BCG bacterial solution (concentration is about 1×10 10 CFU / ml).

[0040] 2. Screening of positive clones

[0041] After electroporation, they were inoculated on a medium (slant) containing 50 μg / ml kanamycin for positive clone selection.

[0042] 3. Detection of target gene expression

[0043] The screened positive clones (ie, recombinant BCG) were inoculated into liquid medium for expansion culture, the culture supernatant was collected, and the expression level...

Embodiment 3

[0044] Effect experiment of embodiment 3 brucellosis vaccines

[0045] Immunize female Balb / c mice aged 6-8 weeks with recombinant BCG and inject subcutaneously at a dose of 4×10 8 CFU / mouse, 4 weeks after immunization, the expression of Th1 / Th2 cytokines in the serum of mice in each group was detected. The experimental results showed that compared with the recombinant BCG carrying the unoptimized L7 / L12 gene (rBCG-L7 / L12(wild)) and the untransformed BCG, the recombinant BCG carrying the codon-optimized L7 / L12 gene (rBCG-L7 / L12(wild)) L7 / L12) can effectively induce the production of Th1 cytokines such as IL-2 and IFN-γ. ( figure 2 )

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Abstract

The invention provides rBCG (bacillus calmette Guerin) capable of expressing a brucella melitensis L7 / L12 gene. The rBCG is established by transferring an expression vector carrying the brucella melitensis L7 / L12 gene optimized by a codon into BCG. Brucellotoxin ribosomal protein L7 / L12 is a T cell antigen. The BCG is vaccine which is commercialized uniquely up to now to prevent tuberculosis. Research proves that the BCG has a remarkable immunologic adjuvant effect and is an exogenous gene expression host with excellent performance and high safety. The brucella melitensis L7 / L12 gene optimized by the codon is expressed by the BCG, so the expression quantity of the L7 / L12 can be increased, as well as the established rBCG vaccine can simulate infection and parasitism characteristics in Brinell bacteria cells and effectively induce a body to generate immune response, also can exert the advantages such as high safety, preparation simplicity and low cost of the BCG serving as the host and the immunologic adjuvant effect of the BCG, and is expected to become a novel brucellosis vaccine.

Description

technical field [0001] The invention relates to the technical fields of genetic engineering and vaccine preparation, in particular to an rBCG expressing the L7 / L12 gene of Brucella melis and its construction method and application. Background technique [0002] Brucellosis, referred to as brucellosis, is a zoonotic infectious disease caused by Brucella infection. Brucella is a facultative intracellular parasite that is highly infectious and pathogenic to humans and mammals. The genus mainly includes 6 species of sheep, cattle, pig and dog. The first 3 species are mainly prevalent in China, among which Brucella melis infection is the most common. The modes of transmission of brucellosis are animal-animal and animal-human. Livestock such as sheep, cattle, and pigs are most susceptible to infection. Infection of animals can lead to inflammation of reproductive organs and fetal membranes, miscarriage, infertility, and various tissue lesions, which greatly increases the chance ...

Claims

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Application Information

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Patent Type & Authority Patents(China)
IPC IPC(8): C12N15/74C12N1/21A61K39/10A61P31/04C12R1/32
CPCA61K39/098A61K2039/523C07K14/23C12N15/74C12N2800/101C12N2800/22
Inventor 石艳春郑源强韩新荣
Owner INNER MONGOLIA MEDICAL UNIV
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